PLoS ONE (Jan 2013)

Structure determination and biochemical characterization of a putative HNH endonuclease from Geobacter metallireducens GS-15.

  • Shuang-yong Xu,
  • Alexandre P Kuzin,
  • Jayaraman Seetharaman,
  • Alice Gutjahr,
  • Siu-Hong Chan,
  • Yang Chen,
  • Rong Xiao,
  • Thomas B Acton,
  • Gaetano T Montelione,
  • Liang Tong

DOI
https://doi.org/10.1371/journal.pone.0072114
Journal volume & issue
Vol. 8, no. 9
p. e72114

Abstract

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The crystal structure of a putative HNH endonuclease, Gmet_0936 protein from Geobacter metallireducens GS-15, has been determined at 2.6 Å resolution using single-wavelength anomalous dispersion method. The structure contains a two-stranded anti-parallel β-sheet that are surrounded by two helices on each face, and reveals a Zn ion bound in each monomer, coordinated by residues Cys38, Cys41, Cys73, and Cys76, which likely plays an important structural role in stabilizing the overall conformation. Structural homologs of Gmet_0936 include Hpy99I endonuclease, phage T4 endonuclease VII, and other HNH endonucleases, with these enzymes sharing 15-20% amino acid sequence identity. An overlay of Gmet_0936 and Hpy99I structures shows that most of the secondary structure elements, catalytic residues as well as the zinc binding site (zinc ribbon) are conserved. However, Gmet_0936 lacks the N-terminal domain of Hpy99I, which mediates DNA binding as well as dimerization. Purified Gmet_0936 forms dimers in solution and a dimer of the protein is observed in the crystal, but with a different mode of dimerization as compared to Hpy99I. Gmet_0936 and its N77H variant show a weak DNA binding activity in a DNA mobility shift assay and a weak Mn²⁺-dependent nicking activity on supercoiled plasmids in low pH buffers. The preferred substrate appears to be acid and heat-treated DNA with AP sites, suggesting Gmet_0936 may be a DNA repair enzyme.